AI Article Synopsis

  • Agonist activation of PPARγ is crucial for fat cell development and improving insulin sensitivity, but mutations in this gene can lead to conditions like lipodystrophy and insulin resistance in humans.
  • Research shows conflicting results in mice models regarding PPARγ's role in insulin sensitivity, which highlights the complexity of translating findings across species.
  • The study introduces a new rat model with a specific PPARγ mutation that reduces fat mass and confirms the importance of both PPARγ alleles for proper fat cell function and insulin sensitivity, stressing the need for careful species selection in research.

Article Abstract

Agonist-induced activation of peroxisome proliferator-activated receptor-γ (PPARγ) stimulates adipocyte differentiation and insulin sensitivity. Patients with heterozygous PPARγ dominant-negative mutation develop partial lipodystrophy and insulin resistance. Inconsistent with this evidence in humans, it was reported that heterozygous PPARγ knockout mice have increased insulin sensitivity and that mice with heterozygous PPARγ dominant-negative mutation have normal insulin sensitivity and improved glucose tolerance. In the context of the interspecies intranslatability of PPARγ-related findings, we generated a PPARγ mutant rat with a loss-of-function mutation (Pparg(mkyo)) without dominant-negative activity by using the ENU (N-ethyl-N-nitrosourea) mutagenesis method. Heterozygous Pparg(mkyo/+) rats showed reduced fat mass with adipocyte hypertrophy and insulin resistance, which were highly predictable from known actions of PPARγ agonists and phenotypes of patients with the PPARγ mutation. This report is the first in our knowledge to clearly demonstrate that both alleles of PPARγ are required for normal adipocyte development and insulin sensitivity in vivo. Furthermore, the study indicates that PPARγ regulates mainly adipocyte number rather than adipocyte size in vivo. The choice of appropriate species as experimental models is critical, especially for the study of PPARγ.

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Source
http://dx.doi.org/10.2337/db15-1422DOI Listing

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